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酿酒酵母中RTF1的鉴定,RTF1是一种对TATA框结合蛋白选择TATA位点很重要的新基因。

Identification of RTF1, a novel gene important for TATA site selection by TATA box-binding protein in Saccharomyces cerevisiae.

作者信息

Stolinski L A, Eisenmann D M, Arndt K M

机构信息

Department of Biological Sciences, University of Pittsburgh, Pennsylvania 15260, USA.

出版信息

Mol Cell Biol. 1997 Aug;17(8):4490-500. doi: 10.1128/MCB.17.8.4490.

Abstract

Interaction of the TATA box-binding protein (TBP) with promoters of RNA polymerase II-transcribed genes is an early and essential step in mRNA synthesis. Previous studies have demonstrated that the rate-limiting binding of TBP to a TATA element can be influenced by transcriptional regulatory proteins. To identify additional factors that may regulate DNA binding by TBP in vivo, we performed a genetic selection for extragenic suppressors of a yeast TBP mutant that exhibits altered and relaxed DNA binding specificity. This analysis has led to the discovery of a previously unidentified gene, RTF1. The original rtf1 suppressor mutation, which encodes a single amino acid change in Rtf1, and an rtf1 null allele suppress the effects of the TBP specificity mutant by altering transcription initiation. Differences in the patterns of transcription initiation in these strains strongly suggest that the rtf1 missense mutation is distinct from a simple loss-of-function allele. The results of genetic crosses indicate that suppression of TBP mutants by mutations in RTF1 occurs in an allele-specific fashion. In a strain containing wild-type TBP, the rtf1 null mutation suppresses the transcriptional effects of a Ty delta insertion mutation in the promoter of the HIS4 gene, a phenotype also conferred by the TBP altered-specificity mutant. Finally, as shown by indirect immunofluorescence experiments, Rtf1 is a nuclear protein. Taken together, our findings suggest that Rtf1 either directly or indirectly regulates the DNA binding properties of TBP and, consequently, the relative activities of different TATA elements in vivo.

摘要

TATA盒结合蛋白(TBP)与RNA聚合酶II转录基因的启动子相互作用是mRNA合成过程中早期且关键的一步。先前的研究表明,TBP与TATA元件的限速结合会受到转录调节蛋白的影响。为了鉴定在体内可能调节TBP与DNA结合的其他因子,我们对酵母TBP突变体的基因外抑制子进行了遗传筛选,该突变体表现出改变且松弛的DNA结合特异性。这项分析导致发现了一个先前未鉴定的基因RTF1。最初的rtf1抑制子突变在Rtf1中编码单个氨基酸变化,而rtf1无效等位基因通过改变转录起始来抑制TBP特异性突变体的作用。这些菌株中转录起始模式的差异强烈表明,rtf1错义突变不同于简单的功能丧失等位基因。遗传杂交结果表明,RTF1中的突变对TBP突变体的抑制以等位基因特异性方式发生。在含有野生型TBP的菌株中,rtf1无效突变抑制了HIS4基因启动子中Tyδ插入突变的转录效应,TBP特异性改变的突变体也赋予了这种表型。最后,如间接免疫荧光实验所示,Rtf1是一种核蛋白。综上所述,我们的研究结果表明,Rtf1直接或间接调节TBP的DNA结合特性,从而调节体内不同TATA元件的相对活性。

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